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Download Genetic Controls in Eukaryotes
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Level of Gene Control in Eukaryotes Chromosome structure and levels of DNA packing DNA is associated with proteins called histones o Nucleosome: DNA is wrapped twice around histones… o Chromatin: nucleosomes ordered in tight spiral… o Chromatin fibers folded in “looped domains”… o more folding and spiraling into final chromosome Regulation of chromatin structure - Histone modification o Histone acetylation (acetyl groups -C0CH3) are attached to + (lysine) histone tails. o When acetylated = neutral and cannot bind to neighboring nucleosomes o No binding = loose structure = easier access to genes for transcription. o Remove these = deacetylation. = inactive genes Regulation of chromatin structure - DNA Methylation o Inactive DNA is highly methylated (-CH3) o Ex. inactive X chromosome in mammalian females = barr bodies Removal of methyl groups = active genes = = genomic imprinting = methylation permanently regulates expression of either maternal or paternal alleles of certain genes at the start of development. o Duel mechanism = = DNA methylation and histone deacetylation can stop transcription. Regulation at transcriptional level - Roles of transcription factors (enhancers & repressors) o To initiate transcription requires transcription factors. o Bind to promoter (TATA box); RNA Pol II can bind o “General” transcription factors leads to slow transcription. - General = essential to initiation of transcription of all protein o “Specific” transcription factors leads to faster transcription = Specific to transcription of particular protein. Regulation at post-transcriptional level - RNA processing o Alternative RNA splicing = different segments of RNA are treated as exons and introns = different mRNA o Controlled by regulatory proteins specific to each cell type o Consequence = a single gene can code for more than one polypeptide = alternative RNA splicing o Humans can have fewer genes than proteins that are made. - mRNA degradation o How long mRNA stays in cytoplasm will determine how much protein synthesis… o Use enzymes to shorten poly-A tail = triggers enzymes to remove 5’ cap = enzymes chew up mRNA (can last minutes to weeks) o Untranslated region near 3’ end (poly-A tail) determine mRNA’s length of longevity. o Another reason,….microRNA’s (miRNAs) o protein + miRNA binds to complementary sequence of mRNA = blocks translation. Regulation at translational level - Initiation of Translation o Regulatory proteins can bind to mRNA at 5’ end preventing initiation of translation (ribosomes can’t attach) o Stored mRNA’s in an egg lack poly-A tails = can’t initiate translation. - At right developmental times, A’s are added so translation can begin - Protein processing and degradation o Proteins have to undergo various chemical modifications before they are activated and functional. - add phosphates to activate = Ex. proton pump - Cell surface protein and others must be transported to a target destination in the cell in order to function o How long protein lasts in a cell…selective degradation - Ex. cyclins = proteins that regulate cell cycle are short lived.